Transgenic plant and the method for producing the same

ABSTRACT

The present invention is directed to a transgenic plant and a method for producing the same. In particular, the present invention is directed to a transgenic plant or a plant cell in which a nucleic acid molecule encoding an m 6 A demethylase is introduced, wherein said m 6 A demethylase has the following two domains: i) N-terminal domain (NTD) having the function of AlkB oxidation demethylase; and ii) C-terminal domain (CTD). The present invention is also directed to a method for producing said plant, comprising introducing a nucleic acid molecule encoding an m 6 A demethylase into a regenarable plant cell, and regenerating a transgenic plant from the regenerable plant cell.

TECHNICAL FIELD

The present invention is directed to a transgenic plant and a method for producing the same. In particular, the present invention is directed to introducing a nucleic acid molecule into a plant to increase the biomass and/or yield of the plant.

INCORPORATION BY REFERENCE OF SEQUENCE LISTING

The instant application contains a sequence listing which has been submitted electronically in XML format and is hereby incorporated by reference in its entirety. Said XML copy, created on May 17, 2023, is named SL.XML and is 34,452 bytes in size.

BACKGROUND

Due to the increasing population in the world, the area of the available earth for agriculture is decreasing. To increase the efficiency of agriculture and increase the diversity of the horticultural plants remains the main object of researches. Conventional methods for improving crops and horticultural plants utilize selective breeding technologies to identify plants with desired properties. This kind of selective breeding technologies, however, has several defects: these technologies are generally labor intensive, and result in plants which generally comprise heterogeneous genetic complements which do not always transfer desired traits from the patent plants.

The development of molecular biology allows people to manipulate animals and plants. The genetic engineering of plants requires isolating and manipulating genetic materials (generally in the form of DNA or RNA) and then introducing genetic materials into plants. Such technology has resulted in plants having a variety of improved economic, agricultural or horticultural traits. A trait having special economic significance is a growth characteristic, for example, high yield.

Yield of seeds is a very important trait, for the seeds of many plants are very important to the nutrition of human being and animals. No matter via the consumption of the seeds per se or that of the meat products based on processed seeds, crops such as maize, rice, wheat and soybean, account for more than half of the total calories taken in by human. They are also origins of sugars, oils and many kinds of metabolites used for industrial processing. Based on the constant need of finding genes for increasing yield of seeds, the prior art has disclosed methods via manipulating hormone levels of plants (WO03/050287), via manipulating cell cycles (WO2005/061702) and manipulating genes involved in salt stress reactions (WO 2004/058980). In addition to yield of seeds, size of a thousand seeds, weight of a single plant, tiller number and/or plant height are also important traits for measuring yield of plants. Moreover, it should be clarified that the growth rate of a plant is not necessarily related to its yield. For example, when the fertilizer is sufficient, rice tends to grow too fast and too high during the early stage and exhibits lodging during the late stage. This leads to the decrease of yield.

Transgenic technologies introduce artificially isolated and modified genes into the genome of an organism, and lead to hereditary modifications of traits of the organism due to the expression of the introduced genes. Researches of transgenic technologies of plants mostly focus on the fields of anti-insect genetic engineering, anti-disease genetic engineering, stress resistance genetic engineering, quality genetic engineering, etc. Transgenic plants which have been commercialized are mainly anti-insect and anti-herbicide varieties. The planting of those varieties decreases the use of chemical pesticides by 37%, increases the yield of crops by 22%, and increases the profit of farmers by 68%. The current transgenic technologies, however, increase the yield indirectly by anti-insect and anti-herbicide properties, etc.

Previous researches on epigenetics generally focus on reversible modifications of DNA and histone. Recently, researchers gradually move their interest to the field of RNA modification. Up to now, scientists have discovered hundreds of RNA modifications N⁶-methyladenoesine (m⁶A) is the most abundant RNA modification in mRNA across all eukaryotes. The modification of m⁶A has been discovered for more than forty years, but its function was not known until the inventor of the present application found the demethylase of m⁶A, FTO protein for the first time (Jia et al, N⁶-methyladenosine in nuclear RNA is a major substrate of the obesity-associated FTO. Nat Chem Biol, 2011, 7 (12): 885-887) , reported the reversibitly of RNA modification for the first time and started the “RNA epigenetics (or Epitranscriptome)” research in 2011. In 2012, researchers developed m⁶A antibody assisted whole transcriptome m⁶A high-throughput sequencing technology, m⁶A-seq (or MeRIP). The result of the sequencing shows that there are about 12,000 m⁶A sites in human and mouse cells, mainly distribute on 7,000 mRNAs transcribed from encoding genes and 300 non-coding RNAs (ncRNAs) transcribed from non-coding genes (Dominissini et al, Topology of the human and mouse m⁶A RNA methylomes revealed by m⁶A-seq. Nature, 2012, 485 (7397): 201-206; Meyer et al, Comprehensive analysis of mRNA methylation reveals enrichment in 3′ UTRs and near stop codons. Cell, 2012, 149 (7): 1635-1646). Up to now, it has been found in the mammalian that the main components of the methyltransferase are METTL3, METTL14 and WTAP (liu et al, A METTL3-METTL14 complex mediates mammalian nuclear RNA N⁶-adenosine methylation. Nat Chem Biol, 2014, 10 (2): 93-95; Ping et al, Mammalian WTAP is a regulatory subunit of the RNA N6-methyladenosine methyltransferase. Cell Res, 2014, 24 (2): 177-189) . There are two kinds of m⁶A demethylases, which are FTO (fat mass and obesity associated) and ALKBH5 (Jia et al, N⁶-methyladenosine in nuclear RNA is a major substrate of the obesity-associated FTO. Nat Chem Biol, 2011, 7 (12): 885-887; Zheng et al, ALKBH5 is a mammalian RNA demethylase that impacts RNA metabolism and mouse fertility. Mol Cell, 2013, 49 (1): 18-29). m⁶A regulates the metabolic processing of mRNAs, including splicing, nuclear export, stability and protein translation via m⁶A binding proteins.

In the plant field, researchers found that mRNAs of all plants comprise m⁶A extensively. It is produced by m⁶A modifying enzymes (currently reported modifying enzyme subunits are classified as MTA (METTL3 homologous gene) and FIP37 (WTAP homologous gene)), and has important regulatory effect on the growth and development of plants. Researchers found that when MTA or FIP37 was knocked out from Arabidopsis thaliana, the seed could not germinated normally. When MTA or FIP37 was partially complemented during the germinating stage, after germinating, the loss of m⁶A from Arabidopsis thaliana severely inhibited the normal growth and development of the plant (Zhong, S., Li, H., Bodi, Z., Button, J., Vespa, L., Herzog, M., and Fray, R. G (2008). MTA is an Arabidopsis messenger RNA adenosine methylase and interacts with a homolog of a sex-specific splicing factor. Plant Cell 20, 1278-1288; Shen, L., Liang, Z., Gu, X., Chen, Y, Teo, Z. W., Hou, X., Cai, W. M., Dedon, P. C., Liu, L., and Yu, H. (2016). N⁶-Methyladenosine RNA Modification Regulates Shoot Stem Cell Fate in Arabidopsis. Dev Cell 38, 186-200).

The inventor of the present application previously found that during the demethylation process of m⁶A in RNA, FTO produced two relatively stable new modifications, hm⁶A (N⁶-hydroxymethyladenosine) and f⁶A (N⁶-formyladenosine), which had potential regulatory effect on RNA processing (Fu et al, FTO-mediated formation of N⁶-hydroxymethyladenosine and N⁶-formyladenosine in mammalian RNA. Nat Commun, 2013, 4 :1798). New experimental data of the inventor showed that FTO could remove tRNA methylation modifications (the data has not been published).

It has been the task of the researches of all agriculture scientists that how to increase the yield of crops in limited area of earth to feed increasing population and how to directly and effectively increase the biomass and yield of plants. For crops (such as rice, wheat, maize), traditional transgenic technologies and hybridization breeding technologies may optimize a certain single gene, and increase the yield by 10%-30%. To achieve extremely high yield, it needs synergetic effects of many genes. The regulation of the metabolic level of mRNA by RNA methylation modification, provides the possibility of a method for regulating a single gene to achieve high yield or increase biomass.

SUMMARY OF THE INVENTION

The inventor has surprisingly found that by introducing m⁶A demethylase FTO into plants, the metabolic level of mRNA may be regulated, and it provides the possibility of a method for regulating a single gene to achieve high yield and/or increase biomass. To efficiently increase the yield and/or biomass of plants, the inventor introduced a heterogenous m⁶A demethylase by transgenic technologies, and dynamically regulate the content of m⁶A in mRNAs of plants so as to regulate the splicing, nuclear export, stability and protein translation of mRNAs. Compared with the traditional hybridization breeding method which increases the yield by 20-30%, with the method of the present invention, the yield of plants increased 4 folds and the biomass increased 4 folds by the regulation of a single gene. It really achieved the high yield and high biomass of plants by the regulation of a single gene.

In particular, the present invention is directed to the following aspects:

In one aspect, the present invention is directed to a transgenic plant or plant cell in which a nucleic acid molecule encoding an m⁶A demethylase is introduced, wherein said m⁶A demethylase has the following two domains:

i) N-terminal domain (NTD) having the function of AlkB oxidation demethylase; and

ii) C-terminal domain (CTD).

In another aspect, the present invention is directed to a method for producing a transgenic plant exhibiting an increased biomass, an increased yield (for example, increased seed/grain yield, increased tuber yield, increased leaf yield, increased stem yield, increased root yield, increased seed cotton yield) or the combination thereof, wherein said method comprises:

a) introducing a nucleic acid molecule encoding an m⁶A demethylase into a regenarable plant cell, wherein said m⁶A demethylase has the following two domains:

-   -   i) N-terminal domain (NTD) having the function of AlkB oxidation         demethylase; and     -   ii) C-terminal domain (CTD); and

b) regenerating a transgenic plant from the regenerable plant cell, wherein the transgenic plant comprises in its genome said nucleic acid molecule encoding the m⁶A demethylase, and exhibits an increased biomass, an increased yield or the combination thereof when compared with a control plant which does not comprise the nucleic acid molecule encoding the m⁶A demethylase.

In one embodiment, said method further comprises:

c) obtaining a progeny plant derived from the transgenic plant of step b), wherein said progeny plant comprises in its genome said nucleic acid molecule encoding the m⁶A demethylase, and exhibits an increased biomass, an increased yield or the combination thereof when compared with a control plant which does not comprise the nucleic acid molecule encoding the m⁶A demethylase.

In one embodiment, the aforesaid m⁶A demethylase is a FTO protein. Said FTO protein is from vertebrates or marine algae.

In one embodiment, said FTO protein has at least 40%, preferably at least 50%, more preferably at least 60%, more preferably at least 70%, more preferably at least 80%, more preferably at least 90%, more preferably at least 95%, more preferably at least 99%, most preferably 100% identity to any one of SEQ ID NOs:1-4.

In one embodiment, said nucleic acid molecule encoding the m⁶A demethylase has at least 90%, preferably at least 95%, more preferably at least 99%, most preferably 100% identity to any one of SEQ ID NOs:5-12.

The transgenic plant of the present invention exhibits an increased biomass, an increased yield or the combination thereof when compared with a control plant which does not comprise the nucleic acid molecule encoding the m⁶A demethylase.

In one embodiment, the plant of the present invention is selected from the group consisting of rice, maize (Zea mays), soybean, tobacco, potato, alfalfa (Medicago sativa), rape (Brassica), Russian dandelion (Taraxacum Kok-saghyz), cotton, wheat, millet (Panicum miliaceum), flax, sunflower and false flax(Camelina sativa)

The present invention is also directed to a tissue, an organ, a pollen, a seed, a grain, a fruit and a progeny plant of the aforesaid transgenic plant.

DESCRIPTION OF THE DRAWINGS AND THE SEQUENCES

FIG. 1 shows the map of pCAMBIA1307 plasmid in which a nucleic acid encoding FTO is introduced.

SEQ ID NO: 1 is the sequence of human (Homo sapiens) FTO protein.

SEQ ID NO: 2 is the sequence of pig (Sus scrofa) FTO protein.

SEQ ID NO: 3 is the sequence of cattle (Bos taurus) FTO protein.

SEQ ID NO: 4 is the sequence of Ostreococcus lucimarinus FTO protein, from a type of marine algae, Ostreococcus lucimarinusn.

SEQ ID NOs: 5 and 6 are nucleic acid sequences encoding human FTO protein. SEQ ID NO:5 is the natural sequence isolated from human, and SEQ ID NO:6 is the sequence which has been codon-optimized for the expression in plants.

SEQ ID NOs: 7 and 8 are nucleic acid sequences encoding pig FTO protein. SEQ ID NO: 7 is the natural sequence isolated from pig, and SEQ ID NO: 8 is the sequence which has been codon-optimized for the expression in plants.

SEQ ID NOs: 9 and 10 are nucleic acid sequences encoding cattle FTO protein. SEQ ID NO: 9 is the natural sequence isolated from cattle, and SEQ ID NO: 10 is the sequence which has been codon-optimized for the expression in plants.

SEQ ID NOs: 11 and 12 are nucleic acid sequences encoding Ostreococcus lucimarinus FTO protein. SEQ ID NO: 11 is the natural sequence isolated from Ostreococcus lucimarinus, and SEQ ID NO: 12 is the sequence which has been codon-optimized for the expression in plants.

DETAILED DESCRIPTION OF THE INVENTION

m⁶A demethylase or the homologs thereof and the nucleic acids encoding said demethylase or the homologs may be used to produce the transgenic plant of the present invention. The m⁶A demethylase used by the present invention may be present in any vertebrates and marine algae. Said enzyme consists of nuclear localization sequence (NLS) and the following two domains: i) N-terminal domain (NTD) having the function of AlkB oxidation demethylase; and ii) C-terminal domain (CTD).

As used herein “homolog” means a protein in a group of proteins that perform the same biological function. Homologs are expressed by homologous genes. Homologous genes include naturally occurring alleles and artificially-created variants. Degeneracy of the genetic code provides the possibility to substitute at least one base of the protein encoding sequence of a gene with a different base without causing the amino acid sequence of the polypeptide produced from the gene to be changed. Homologs are proteins that, when optimally aligned, have at least 40% identity, more preferably about 50% or higher, more preferably about 60% or higher, more preferably about 70% or higher, more preferably at least 80% and even more preferably at least 90% identity over the full length of a protein identified as increasing the yield and/or biomass of plants when expressed in plant cells.

Homologs are be identified by comparison of amino acid sequence, e.g. manually or by use of a computer-based tool using known homology-based search algorithms such as those commonly known and referred to as BLAST, FASTA, and Smith-Waterman. A local sequence alignment program, e.g. BLAST, can be used to search a database of sequences to find similar sequences, and the summary Expectation value (E-value) used to measure the sequence base similarity. As a protein hit with the best E-value for a particular organism may not necessarily be an ortholog or the only ortholog, a reciprocal query is used in the present invention to filter hit sequences with significant E-values for ortholog identification. The reciprocal query entails search of the significant hits against a database of amino acid sequences from the base organism that are similar to the sequence of the query protein. A hit is a likely ortholog, when the reciprocal query's best hit is the query protein itself or a protein encoded by a duplicated gene after speciation. A further aspect of the invention comprises functional homolog proteins that differ in one or more amino acids from those of disclosed protein as the result of conservative amino acid substitutions, for example substitutions are among: acidic (negatively charged) amino acids such as aspartic acid and glutamic acid; basic (positively charged) amino acids such as arginine, histidine, and lysine; neutral polar amino acids such as glycine, serine, threonine, cysteine, tyrosine, asparagine, and glutamine; neutral nonpolar (hydrophobic) amino acids such as alanine, leucine, isoleucine, valine, proline, phenylalanine, tryptophan, and methionine; amino acids having aliphatic side chains such as glycine, alanine, valine, leucine, and isoleucine; amino acids having aliphatic-hydroxyl side chains such as serine and threonine; amino acids having amide-containing side chains such as asparagine and glutamine; amino acids having aromatic side chains such as phenylalanine, tyrosine, and tryptophan; amino acids having basic side chains such as lysine, arginine, and histidine; amino acids having sulfur-containing side chains such as cysteine and methionine; naturally conservative amino acids such as valine-leucine, valine-isoleucine, phenylalanine-tyrosine, lysine-arginine, alanine-valine, aspartic acid-glutamic acid, and asparagine-glutamine. A further aspect of the homologs encoded by DNA useful in the transgenic plants of the invention are those proteins that differ from a disclosed protein as the result of deletion or insertion of one or more amino acids in a native sequence.

As used herein, “percent identity” means the extent to which two optimally aligned DNA or protein segments are invariant throughout a window of alignment of components, for example nucleotide sequence or amino acid sequence. An “identity fraction” for aligned segments of a test sequence and a reference sequence is the number of identical components that are shared by sequences of the two aligned segments divided by the total number of sequence components in the reference segment over a window of alignment which is the smaller of the full test sequence or the full reference sequence. “Percent identity” (“% identity”) is the identity fraction times 100.

The m⁶A demethylase used in the present invention may be SEQ ID NO: 1, 2, 3 or 4 of the homolog thereof. Said homolog has at least 40%, 41%, 42%, 43%, 44%, 45%, 46%, 47%, 48%, 49%, 50%, 51%, 52%, 53%, 54%, 55%, 56%, 57%, 58%, 59%, 60%, 61%, 62%, 63%, 64%, 65%, 66%, 67%, 68%, 69%, 70%, 71%, 72%, 73%, 74%, 75%, 76%, 77%, 78%, 79%, 80%, 81%, 82%, 83%, 84%, 85%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, or 99% sequence identity to any one of SEQ ID NOs: 1-4.

The nucleic acid encoding the m⁶A demethylase used in the present invention may be any one of SEQ ID NOs: 5-12 or the homologous gene thereof. Said homologous gene has at least 40%, 41%, 42%, 43%, 44%, 45%, 46%, 47%, 48%, 49%, 50%, 51%, 52%, 53%, 54%, 55%, 56%, 57%, 58%, 59%, 60%, 61%, 62%, 63%, 64%, 65%, 66%, 67%, 68%, 69%, 70%, 71%, 72%, 73%, 74%, 75%, 76%, 77%, 78%, 79%, 80%, 81%, 82%, 83%, 84%, 85%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, or 99% sequence identity to any one of SEQ ID NOs: 5-12.

The nucleic acid encoding the m⁶A demethylase defined herein may not be a full-length nucleic acid. A part of the nucleic acid encoding the m⁶A demethylase defined herein may be prepared by making one or more deletions from the full-length nucleic acid.

Another nucleic acid variant used in the present invention is a nucleic acid which hybridizes with the nucleic acid encoding the m⁶A demethylase defined herein or with a part of the nucleic acid encoding the m⁶A demethylase defined herein under stringent conditions.

Appropriate stringent conditions which promote DNA hybridization are, for example, 6.0×sodium chloride/sodium citrate (SSC) at about 45° C., followed by a wash of 2.0 ×SSC at 50° C., are known to those skilled in the art or can be found in Current Protocols in Molecular Biology (1989). For example, the salt concentration in the wash step can be selected from a low stringency of about 2.0×SSC at 50° C. to a high stringency of about 0.2×SSC at 50° C. In addition, the temperature in the wash step can be increased from low stringency conditions at room temperature, about 22° C., to high stringency conditions at about 65° C. Both temperature and salt may be varied, or either the temperature or the salt concentration may be held constant while the other variable is changed. The nucleic acid used in the present invention may specifically hybridize with a nucleic acid encoding a FTO protein, for example, any one of SEQ ID NOs: 5-12 or a part thereof under said conditions.

All or a portion of the nucleic acids of the present invention may be synthesized using codons preferred by a selected host. Species-preferred codons may be determined, for example, from the codons used most frequently in the proteins expressed in a particular host species. Therefore, the nucleic acids of the present invention include those obtained by making codon-optimization to natural FTO proteins for the expression in plants. Other modifications of the nucleotide sequences may result in mutants having slightly altered activity.

The present invention is directed to a transgenic plant in which a gene encoding the aforesaid m⁶A demethylase FTO or a homolog thereof is introduced, or a progeny plant thereof. The present invention is also directed to a cell, a tissue, an organ, a pollen, a seed, a grain or a fruit of said plant.

“Introduced” in the context of inserting a nucleic acid fragment (e.g., a recombinant DNA construct) into a cell, means “transfection” or “transformation” or “transduction” and includes reference to the incorporation of a nucleic acid fragment into a eukaryotic or prokaryotic cell where the nucleic acid fragment may be incorporated into the genome of the cell (e.g., chromosome, plasmid, plastid or mitochondrial DNA), converted into an autonomous replicon, or transiently expressed (e.g., transfected mRNA).

“Plant” includes reference to whole plants, plant organs, plant tissues, seeds and plant cells and progeny of same. Plant cells include, without limitation, cells from seeds, suspension cultures, embryos, meristematic regions, callus tissue, leaves, roots, shoots, gametophytes, sporophytes, pollen, and microspores. “Progeny” comprises any subsequent generation of a plant.

According to the use, the plants of the present invention may be food crops, economic crops, vegetable crops, fruits, flowers, grasses, trees, industrial raw material crops, feed crops or medicine crops. Specifically, said food crops include rice, maize, soybean, beans, yams, potato, hulless barley, broad bean, wheat, barley, millet, rye, oat, sorghum, etc.; Said economic crops include oil tea, rape, rapeseed, flax, false flax(Camelina sativa), peanut, oil flax (Linum usitatissimum), mariguana (Cannabis sativa) , sunflower, tobacco, cotton, beet, sugarcane, etc.; said vegetable crops include radish, Chinese cabbage, tomato, cucumber, hot pepper, carrot, etc.; said fruits include pear, apple, walnut, cherry, strawberry, jujube or peach; said flowers include flowers for view, for example, orchid, chrysanthemum, carnation, rose, green plants, etc., said grasses and trees include populus, hevea brasiliensis, taxus chinensis, and those for urban greening or those living in deserts and harsh conditions such as drought; said industrial raw material crops include Russian dandelion, guayule, jatropha curcas, etc., said feed crops include the foodstuff for livestock, such as alfalfa etc.; said drug crops include ginseng, angelica and ganoderma, etc..

“Transgenic plant” includes reference to a plant which comprises within its genome a heterologous polynucleotide. Preferably, the heterologous polynucleotide is stably integrated within the genome such that the polynucleotide is passed on to successive generations. The heterologous polynucleotide may be integrated into the genome alone or as part of a recombinant DNA construct. “Heterologous” with respect to sequence means a sequence that originates from a foreign species, or, if from the same species, is substantially modified from its native form in composition and/or genomic locus by deliberate human intervention.

The present invention has prepared a DNA construct which comprises a nucleic acid molecule encoding the FTO protein described herein. The construct may comprise the nucleic acid molecule encoding the FTO protein described herein optionally operably linked to a promoter sequence which functions in a host cell. Other construct components may include additional regulatory elements, such as 5′ leaders and introns for enhancing transcription, 3′ untranslated regions (such as polyadenylation signals and sites), DNA for transit, signal peptides, or one or more selective maker genes.

As used herein, “promoter” means regulatory DNA for initializing transcription. A plant promoter is a promoter capable of initiating transcription in plant cells whether or not its origin is a plant cell, e.g. is it well known that Agrobacterium promoters are functional in plant cells. Thus, plant promoters include promoter DNA obtained from plants, plant viruses and bacteria such as Agrobacterium and Bradyrhizobium bacteria. Examples of promoters under developmental control include promoters that preferentially initiate transcription in certain tissues, such as leaves, roots, or seeds. Such promoters are referred to as “tissue preferred”. Promoters that initiate transcription only in certain tissues are referred to as “tissue specific”. A “cell type” specific promoter primarily drives expression in certain cell types in one or more organs, for example, vascular cells in roots or leaves. An “inducible” or “repressible” promoter is a promoter which is under environmental control. Examples of environmental conditions that may affect transcription by inducible promoters include anaerobic conditions, or certain chemicals, or the presence of light. Tissue specific, tissue preferred, cell type specific, and inducible promoters constitute the class of “non-constitutive” promoters. A “constitutive” promoter is a promoter which is active under most conditions. Promoters useful in the present invention are not specifically limited. Those skilled in the art may select suitable promoters according to their knowledge.

As used herein “operably linked” means the association of two or more DNA fragments in a DNA construct so that the function of one, e.g. protein-encoding DNA, is controlled by the other, e.g. a promoter.

The DNA construct generally contain a selective maker gene. Selective marker genes are used to provide an efficient system for identification of those cells that are stably transformed by receiving and integrating a transgenic DNA construct into their genomes. Preferred marker genes provide selective markers which confer resistance to a selective agent, such as an antibiotic or herbicide. Potentially transformed cells are exposed to the selective agent. In the population of surviving cells will be those cells where, generally, the resistance-conferring gene is integrated and expressed at sufficient levels to permit cell survival. Cells may be tested further to confirm stable integration of the exogenous DNA. Commonly used selective marker genes include those conferring resistance to antibiotics such as kanamycin and paromomycin (nptII), hygromycin B (aph IV) and gentamycin (aac3 and aacC4) or resistance to herbicides such as glufosinate (bar or pat) and glyphosate (aroA or EPSPS). Examples of such selective markers are illustrated in U.S. Pat. Nos. 5,550,318; 5,633,435; 5,780,708 and 6,118,047, all of which are incorporated herein by reference. Selectvie markers which provide an ability to visually identify transformants can also be employed, for example, a gene expressing a colored or fluorescent protein such as a luciferase or green fluorescent protein (GFP) or a gene expressing a beta-glucuronidase or uidA gene (GUS) for which various chromogenic substrates are known.

The introduction of the recombinant DNA construct into plants may be carried out by any suitable technique, including but not limited to direct DNA uptake, chemical treatment, electroporation, microinjection, cell fusion, infection, vector mediated DNA transfer, bombardment, or Agrobacterium mediated transformation. For Agrobacterium tumefaciens based plant transformation system, additional elements present on transformation constructs will include T-DNA left and right border sequences to facilitate incorporation of the recombinant polynucleotide into the plant genome.

In general it is useful to introduce recombinant DNA randomly, i.e. at a non-specific location, in the genome of a target plant line. In special cases it may be useful to target recombinant DNA insertion in order to achieve site-specific integration, for example to replace an existing gene in the genome, to use an existing promoter in the plant genome, or to insert a recombinant polynucleotide at a predetermined site known to be active for gene expression. Several site specific recombination systems exist which are known to function in plants include cre-lox as disclosed in U.S. Pat. No. 4,959,317 and FLP-FRT as disclosed in U.S. Pat. No. 5,527,695, both incorporated herein by reference.

Transformation methods of this invention are preferably practiced in tissue culture on media and in a controlled environment. “Media” refers to the numerous nutrient mixtures that are used to grow cells in vitro, that is, outside of the intact living organism. Recipient cell targets include, but are not limited to, meristem cells, callus, immature embryos and gametic cells such as microspores, pollen, sperm and egg cells. It is contemplated that any cell from which a fertile plant may be regenerated is useful as a recipient cell. Callus may be initiated from tissue sources including, but not limited to, immature embryos, seedling apical meristems, microspores and the like. Cells capable of proliferating as callus are also recipient cells for genetic transformation. Practical transformation methods and materials for making transgenic plants of this invention, for example various media and recipient target cells, transformation of immature embryo cells and subsequent regeneration of fertile transgenic plants are disclosed in U.S. Pat. Nos. 6,194,636 and 6,232,526, which are incorporated herein by reference.

The development or regeneration of plants containing the foreign, exogenous isolated nucleic acid fragment that encodes a protein of interest is well known in the art. The regenerated plants are self-pollinated to provide homozygous transgenic plants. Otherwise, pollen obtained from the regenerated plants is crossed to seed-grown plants of agronomically important lines. Conversely, pollen from plants of these important lines is used to pollinate regenerated plants. A transgenic plant of the present invention containing the nucleic acid molecule encoding the FTO protein is cultivated using methods well known to one skilled in the art.

The seeds of transgenic plants can be harvested from fertile transgenic plants and be used to grow progeny generations of transformed plants of this invention including hybrid plants line for selection of plants having an enhanced trait. In addition to direct transformation of a plant with the nucleic acid molecule encoding the FTO protein, transgenic plants can be prepared by crossing a first plant having the nucleic acid molecule encoding the FTO protein with a second plant lacking the nucleic acid molecule. For example, the nucleic acid molecule encoding the FTO protein can be introduced into first plant line that is amenable to transformation to produce a transgenic plant which can be crossed with a second plant line to introgress the nucleic acid molecule encoding the FTO protein into the second plant line. The transgenic plant derived from the plant cell of the present invention is cultivated to produce increased yield and/or biomass compared with a control plant. As used herein a “control plant” means a plant that does not contain the nucleic acid molecule encoding the FTO protein. A control plant is to identify and select a transgenic plant that has increased yield and/or biomass. A suitable control plant can be a non-transgenic plant of the parental line used to generate a transgenic plant, i.e. devoid of the nucleic acid molecule encoding the FTO protein. A suitable control plant may in some cases be a progeny of a hemizygous transgenic plant line that does not contain the nucleic acid molecule encoding the FTO protein, known as a negative segregant.

The “yield” of the transgenic plant described herein means the harvest amount of the product desired by the cultivation. The standards for evaluating the yields of different plants are different. For example, the subject of the evaluation of the yields of cereal crops (rice, wheat, maize, etc.), beans and oil crops (soybean, peanut, rape, etc.) is the seed (grain); that of cotton is the seed cotton or the lint cotton; that of yam crops (sweet potato, potato, cassava, etc.) is the tuberous root or tuber; that of bast fiber crops is the fiber of stems or the fiber of leaves; that of sugarcane is the stem; that of beet is the root; that of tobacco is the leaf; that of green manure crops (alfalfa, trefoil, etc.) is the stem and leaf, etc. The meaning of the yield of the same plant differs when it is cultivated for different purposes. For example, when maize is cultivated as food and fine feed crop, the yield is the harvest amount of grains, and when it is cultivated as silage, the yield includes the total harvest amount of stems, leaves and ears. The increased yield of the transgenic plant of the present invention may be measured by many means, including measuring weight, seed number per plant, seed weight, tuber weight, seed number per unit area (i.e. seeds, or weight of seeds, per acre), bushels per acre, tonnes per acre, tons per acre, kilo per hectare.

Those skilled in the art can determine the meaning of the yield for each plant and the standard for evaluating it according to the knowledge in the art.

Biomass means the total mass of the existing organic materials of an organism. It is expressed as dry weight, fresh weight, tiller number, etc. in the present invention. The increased biomass of the transgenic plant of the present invention may be measured by many means, including measuring weight, dry weight or fresh weight of the overground parts per plant, tiller number, dry weight of the overground parts per unit area (i.e. dry weight or fresh weight, per acre), bushels per acre, tonnes per acre, tons per acre, kilo per hectare.

EXAMPLES

The present invention is further illustrated in the following Examples. It should be understood that these Examples, while indicating embodiments of the invention, are given by way of illustration only. From the above discussion and these Examples, one skilled in the art can ascertain the essential characteristics of this invention, and without departing from the spirit and scope thereof, can make various changes and modifications of the invention to adapt it to various usages and conditions. Furthermore, various modifications of the invention in addition to those shown and described herein will be apparent to those skilled in the art from the foregoing description. Such modifications are also intended to fall within the scope of the appended claims.

The materials used in the following examples were as follows:

-   -   1. Formulation of YEP broth for the growth of Agrobacterium (per         liter): yeast extract 10 g/L+peptone 10 g/L+NaCl 5 g/L, PH 7.2.         For the solid medium, 15 g/L agar was added.     -   2. Agrobacterium re-suspension AAM broth: 50 ml 20×AA         macroelement, 10 ml 100×FeEDTA, 10 ml 100×B5 macroelement, 10 ml         100×B5 vitamin, 100 ml 10×AA amino acid, 1 ml 100 mM         acetosyringone, 68.5 g sucrose, 36 g glucose, 0.5 g hydrolyzed         casein. The volume was adjusted to 1000 ml. The pH was adjusted         to 5.2. Sterilized with a 0.2 mm cellulose acetate membrane.     -   3. 20×AA macroelement: 59 g KCl, 3 g CaCl₂·2H₂O, 10 g MgSO₄·7H₂O         and 3 g NaH₂PO₄·H₂O. The volume was adjusted with distilled         water to 1 L. Stored at 4° C.     -   4. 10×AA amino acid: 8.76 g Gln, 2.66 g Asp, 1.74 g Arg and 75         mg Gly. The volume was adjusted with distilled water to 1 L.         Sterilized with a 0.2 mm cellulose acetate membrane. Stored at         4° C.     -   5. 10 ml 100×B5 vitamin: 10 g myoinositol, 1 g thiamine         hydrochloride, 100 mg pyridoxine hydrochloride and 100 mg         nicotinic acid. The volume was adjusted with distilled water to         1 L. Stored at 4° C.     -   6. 100×B5 macroelement: 1.320 mg MnSO₄·4H₂O, 200 mg ZnSO₄·7H₂O,         2.5 mg CuSO₄·5H₂O, 25 mg Na₂MoO₄·2H₂O, 2.5 mg CoCl₂·6H₂O, 300 mg         H₃BO₃ and 75 mg KI. The volume was adjusted with distilled water         to 1 L. Stored at 4° C.     -   7. NB medium: macroelements and microelements of N6 medium,         organic elements of B5 medium, 300 mg/L hydrolyzed casein, 500         mg/L glutamine, 30 g/L sucrose and 8 g/L agar.

Example 1: obtaining cDNA of the m⁶A demethylase gene

The FTO genes were searched from the database of National Center for Biotechnology Information (NCBI). Amino acid sequences (SEQ ID NOs: 1-4) and nucleic acid sequences (SEQ ID NOs: 5, 7, 9 and 11) of human (Homo sapiens) FTO, pig (Sus scrofa) FTO, cattle (Bos Taurus) FTO and alga (Ostreococcus lucimarinus CCE9901) FTO were obtained. The corresponding cDNAs were purchased, or synthesized by GenScript when there are no commercialized cDNAs. The amino acid sequences of SEQ ID NOs: 1-4 were optimized to plant codons to synthesize the codon-optimized nucleic acid sequences SEQ ID NOs: 6, 8, 10 and 12.

The FTO gene cDNAs used in the following examples are SEQ ID NO:5, 7, 9 and 11.

Example 2: cloning the m⁶A demethylase gene

The FTO gene cDNAs (SEQ ID NO:5, 7, 9, 11) were cloned into the plant binary vector pCAMBIA1307. The average size of the inserted gene sequences was 1.5 kb. The obtained plasmid is shown in FIG. 1 .

Example 3: transformation of the plants

3.1 Introduction of the FTO gene of example 2 into rice with the transgenic technologies

I. Inducing calluses with mature embryos of rice as test materials

1. Sterilization

Mature seeds of rice (japonica Nipponbare) were artificially unshelled. Seeds which were full, bright and clean, and bacterial plaque free were selected and placed into a 100 ml sterilized flask. 70% alcohol was added into the flask to sterilize for 2 minutes. Then, the alcohol was decanted, and 20% NaClO was added to soak for 30 minutes. Then, the NaClO was decanted, and the seeds were rinsed 4-5 times with sterilized distilled water. Lastly, the seeds were soaked with sterilized distilled water for 30 minutes.

2. Introduction culture (under aseptic conditions):

The sterilized seeds were placed on sterilized filter paper. After the water on the surface were absorbed by the filter paper, the seeds were placed into NB medium (PH5.8) containing 2.0 mg/L 2, 4-D at the density of 12-14 seeds per petri dish. To ensure good induction rate, the germination orientation of the seeds was made parallel to the medium or slightly downward, and not upward or vertically upward. Then, the petri dish was sealed with membrane, and was induced and incubated for 20-30 days in an incubator with light at 30° C., 50% humidity until obviously loose calluses appeared. Then, subculture was performed.

3. Subculture (under aseptic conditions):

The petri dish was opened on a super-clean operating desk. Calluses which naturally divided, grew vigorously and which were hard and bright yellow and which had the diameter of about 3 mm were placed in NB medium (PH5.8) containing 2.0 mg/L 2,4-D and 0.5 mg/L 6-BA at the density of 10 calluses per petri dish, and were dark incubated at 30° C. If the calluses seriously turned soft, they were moved into light to be subcultured. The subculture was performed twice, each 10-15 days (the time of the next subculture was determined according to how much the calluses grew).

II. The culture of the Agrobacterium

The pCAMBIA1307 vector carrying FTO gene and Hygromycin resistance gene shown in FIG. 1 was transfected into Agrobacterium LBA4404. Then, Agrobacterium LBA4404 was seeded into YEP solid medium containing 20 mg/L Rifampin (Rif) and 50 mg/L kanamycin (Kan). After cultured at 28° C. for two days, Agrobacterium monoclones were picked up to be subject to colony PCR to test whether the FTO was transferred into the Agrobacterium. Positive monoclones were selected and placed in 4 ml YEP (containing 50 mg/L Kan and 20 mg/L Rif) broth, and were shaking-cultured at 28° C., 220 rpm for 20-36 h until the OD₆₀₀ of the bacterial solution was 0.8˜1.0.

III. Infection and co-culture

-   -   1. The solution of the cultured Agrobacterium was centrifuged at         4° C., 4000 rmp for 10 min, and was made to suspension with AAM         broth containing 100 μmol/L acetosyringone. The final OD₆₀₀ of         the bacterial solution was about 0.2.     -   2. The calluses with certain size was picked up and placed into         the suspension of the Agrobacterium to be infected for 20-30         min.     -   3. The calluses were took out and placed on sterilized filter         paper to be dried for 20-30 min so as to prevent undue injury of         the calluses caused by the over-growth of the Agrobacterium         during the co-culture.     -   4. The calluses were placed in NB medium (PH5.2) containing 2.0         mg/L 2,4-D and 100 μmol/L acetosyringone and were cultured at         25° C. for 48-72 h in the dark.

IV. Screening of calluses with resistance

The calluses were took out and rinsed with shaking by sterilized water for 5-6 times. Then, the calluses were placed on sterilized filter paper to be dried and then placed evenly in NB medium (PH 5.8) containing 50 mg/L hygromycin for the first screening. The calluses were cultured in the dark at 28° C. and when there was growth of mold or Agrobacterium, the calluses were timely moved to a new screening plate.

After screening for about 30 days, new calluses were produced. They were moved to new NB medium (PH 5.8) containing 50 mg/L hygromycin for another 7-10 day screening. If the growth was obvious, they were positive calluses. If there was no growth (even if there was no browning or death), they were possibly false positive.

V. Introducing the differentiation of the calluses with resistance and rooting

The vigorously grew, yellow calluses after the second screening (to ensure that the calluses used to differentiate were not defective) were placed in NB medium (PH 5.8) containing 2.0 mg/L 6-BA, 0.5 mg/L kinetin, and 50 mg/L hygromycin at the density of 2-3 positive clones per bottle. It was enough to place a little of calluses per clone. The placed calluses should have high quality rather than large number. After cultured at 27° C. in the dark for 10 days, they were allowed to differentiate in the light for 10-20 days. After green leaves appeared, they were allowed to root at the light density of 4000lux, 14 h/d.

The strong seedlings differentiated from each clone were placed in 1/2N6 medium (PH5.8) containing 0.5 mg/L naphthaleneacetic acid and 50 mg/L hygromycin to induce rooting at the density of 2-3 seedlings each bottle. The seedlings were cultivated at 27-30° C. in the light at the light density of 4000lux, 14 h/d. After 7-10 days, the sealing membranes were opened to add appropriate amount of water. After 2-3 days, the seedlings were transplanted.

VI. Training and transplantation of the transgenic seedlings

The rice seedlings with well differentiated roots, stems and leaves were picked up (when the seedlings grew to the top of the test tubes, the covers should be opened timely). The sealing membranes were opened and appropriate amount of distilled water or sterilized water was added (to prevent the growth of bacteria in the medium). The seedlings were trained for about 3 days to one week. After the agar was rinsed, the seedlings were transplanted into earthen bowls in the greenhouse to grow and to be tested.

Example 4 Test of the transformed seedlings

-   -   1. PCR detection: The design of FTO gene primers

Primers for detecting human FTO (hFTO):

hFTO-F: 5′-ATGAAGCGCACCCCGACTG-3′ (SEQ ID NO:13);

hFTO-R: 5′-GGGTTTTGCTTCCAGAAGCTGA-3′ (SEQ ID NO:14);

Primers for detecting cattle FTO (cFTO):

cFTO-F: 5′-ATGAAGCGGACCCCGACG-3′ (SEQ ID NO:15);

cFTO-R: 5′-GGGCCTGGTTTCCAGAAGCAG-3′ (SEQ ID NO:16);

Primers for detecting pig FTO (pFTO):

pFTO-F: 5′-ATGAAGCGAACCCCAACCGC-3′ (SEQ ID NO:17);

pFTO-R: 5′-GGGTTTGGCTTCCAGAAGCAGAC-3′ (SEQ ID NO:18);

Primers for detecting Ostreococcus lucimarinus FTO (olFTO):

olFTO-F: 5′-ATGTCGCCGTCATCCTCCG-3′ (SEQ ID NO:19);

olFTO-R: 5′-CACTTTGTTTTGCTCCTCCTCGAGAAA-3′ (SEQ ID NO:20).

The PCR reaction program was: 35 cycles of 95° C. 5 min, 95° C. 15 s, 58° C. 15 s, 72° C. Extended at 72° C. for 10 min, stored at 4° C. After the reaction, PCR products were subject to 1% agarose gel electrophoresis analysis.

-   -   2. Method for rapidly detecting the transgenic seedlings: the         freshly green leaves of about 1 cm were cut and collected from         the seedlings to be tested (both sides had incisions) and were         placed flatly on the test medium (0.7% agar, 1 ml/L 6-BA, 50         mg/L hygromycin) and were cultured at 28° C. for 48 h (16 h         light/8 h dark each day). The plants which have freshly green         leaves were positive ones while the leaves of the negative         seedlings had plaques of necrosis.

Example 5 Evaluation of the effects of FTO genes from several species in rice

The test results of the rice of example 3 are shown in table 1 (the japonica Nipponbare variety which had not been introduced the FTO gene was the control). The data were obtained from 50 transgenic and control rice plants in maturation stage. Dry weight was weighed after placed in 105° C. oven for 20 mins and 80° C. oven for 20 hours.

TABLE 1 Evaluation of the effects of human, cattle, pig and Ostreococcus lucimarinus FTOs introduced into rice (transgenic plants/control plants) The Fresh Dry Biomass of Biomass Biomass introduced Tiller weight of weight of the whole plant (fresh weight of the (dry weight of the nucleic acids number the seeds the seeds (seeds plus the overground parts after overground parts after encoding the Increased Increased Increased overground parts) removing the seeds) removing the seeds) FTOs Plant folds folds folds Increased folds Increased folds Increased folds Human FTO rice 2.54 4.58 4.15 2.61 2.41 3.87 (SEQ ID NO: 5) Cattle FTO 2.15 4.15 3.71 2.37 2.22 3.61 (SEQ ID NO: 7) Pig FTO 2.08 4.02 3.62 2.34 2.11 3.60 (SEQ ID NO: 9) Ostreococcus 1.85 3.78 3.41 2.51 2.15 3.45 lucimarinus FTO (SEQ ID NO: 11)

Table 1 shows that after the nucleic acids encoding the FTOs of several species were introduced to rice, the biomass and the yield of seeds were increased.

The inventor also tested the codon-optimized nucleic acids encoding the FTOs (SEQ ID NOs:6, 8, 10 and 12) by the same method. The data are similar to the above, and thus are not shown herein.

Example 6 Evaluation of the effect of FTO in a variety of plants

A variety of plants were transformed with the nucleic acid encoding human FTO (SEQ ID NO:5) to obtain a variety of transgenic plant cells and plants in which the nucleic acid encoding the FTO were introduced. The methods are as follows:

Genetic Transformation Method of Tobacco

1. Experimental materials

Materials: Tobacco variety: K326; Agrobacterium: LBA4404; HF (human FTO) gene was cloned into the 35S promoter-driven vector pCAMBIA2300. The screened resistance in eukaryotic plants was resistance to Kanamycin.

Chemicals: MS macroelements, MS microelements, MS iron salts, indole acetic acid (IAA), 6-benzylaminoadenine (6-BA), inositol nicotinate (B₁B₆), sucrose, agar, cephalosporin (Cef), carbenicillin (Carb), kanamycin (Kn), gentamicin, rifampicin;

MS medium (1 L): macroelements (20×) 50 ml, microelements (100×) 10 ml, Fe²⁺ (100×) 10 ml, sucrose 30 g, agar 8 g. The pH was about 6.0.

Pre-culture medium (1 L): macroelements (20×) 50 ml, microelements (100×) 10 ml, Fe²⁺ (100×) 10 ml, 6-BA (1000×) 2 ml, B₁B₆ (200×) 5 ml, glycine (1000×) 1 ml, agar 8 g. The pH was about 6.0. After high temperature sterilization, IAA (0.2 mg/L) 1 ml was added.

Differentiation culture medium (1 L): based on the pre-culture medium, cephalosporin 2 ml, carbenicillin 1 ml and kanamycin 1 ml were added.

Rooting culture medium (1 L): 1/2MS, IAA 2 mg/L, sucrose 30 g/L, agar 5.8 g/L, pH=5.8

LB broth (1 L): tryptone 10 g, yeast extract 5 g, NaCl 10 g.

MS₀ medium: MS culture medium without the addition of agar and only containing macroelements

2. Tobacco transformation (Leaf disc method) Tobacco was transformed by leaf disc method. The cut tobacco leaf discs were placed on the pre-culture medium for 1-2 days, and then soaked in Agrobacterium suspension (MS₀ suspended, diluted by 50-100 times) for 3-5 minutes. Then, the discs were taken out, and sterile filter paper was used to absorb the liquid on their surfaces. The infected leaf discs were respectively inoculated on a pre-culture medium covered with two layers of filter paper and cultured at 26° C. for 20-24 h in dark. The discs were rinsed with the sterilized water added with cephalosporin and carbenicillin (1000 times the mother liquor) for 10 min. The, they were finally rinsed with sterilized water for 10 min. Subsequently, sterile filter paper was used to absorb the liquid on their surfaces, and then the discs were placed in the differentiation culture medium for differentiation culture. In the early stages, subculturing was performed every 2-3 says, and each subculturing shall be carried out under aseptic conditions; after the continual subculturing for three times, subculturing was performed every two weeks. Co-culture was carried out until the first bud appeared. The buds were transferred into tissue culture vessels for culturing. When the buds grew to 2 cm, all the calluses at basal parts of buds and basal leaves were cut on a super-clean operating desk, and then the buds were placed in the rooting culture medium. When the roots grew to 3 cm, sterile seedlings were taken out; the solid culture medium was smashed gently, while the residual culture medium was rinsed off. Thereafter, the sterile seedlings were placed in soil, covered with clear plastic bags (pricked), and cultured for about one week, and then transferred outdoors (growing in dark in the first 3 days).

Transformation Method of Potato

1. Materials:

Potato variety: Dongnong 303; Agrobacterium: LBA4404; HF (human FTO) gene was cloned into the 35S promoter-driven vector pCAMBIA2300. The screened resistance in eukaryotic plants was resistance to Kanamycin.

2. Potato transformation

The potatoes were cleaned by rinsing with distilled water, soaked with 75% alcohol for 30 sec, soaked with 0.1% mercuric chloride for 10 min, cleaned with sterilized water for 5 times, and then peeled to be cut into slices with the thicknesses around 1 mm. The slices were mixed with the Agrobacterium solution under gentle shaking to enable the Agrobacterium solution to contact with the explants sufficiently. Sterile filter paper was used to absorb the redundant Agrobacterium solution. Then the potato pieces were placed in the co-culture medium for dark culture. After the completion of co-culture, the potato pieces were cleaned for 3 times with sterilized water and liquid MS culture medium respectively. The redundant Agrobacterium solution was rinsed off. The potato pieces were transferred into the regeneration culture medium. Then, the potato pieces were transferred into the rooting culture medium till the buds grew to 1.5-2.0 mm and were cut, for rooting screening propagation.

Genetic Transformation of Soybean

1. Materials

Agrobacterium strain was LBA4404; somatic cell embryo masses of soybean Dongnong L13 at the globular stage; the transgenic plasmid was a 35S promoter-driven vector pCAMBIA2300 into which the HF gene was cloned. The screened resistance in eukaryotic plants was resistance to kanamycin.

Plant tissue culture medium and culture conditions:

Subculture medium: MS+15 mg/L)−20 mg/L 2,4-D+0.8% agar+3% sucrose pH=5.8 natural light

Re-suspension culture medium: subculture medium (liquid)+AS (0-100 μmol/L) pH=5.8 Natural light

Co-culture medium: infection culture medium+AS (0-100 μmol/L) pH=5.6

Sterilization screening culture medium: subculture medium+(50-300 mg/L) cephalosporin+25-50 mg/L kanamycin

Germination culture medium 1: MS+1% activated carbon+0.8% agar+10% sucrose illumination 16 h/d

Germination culture medium 2: MS+0.8% agar+10% sucrose illumination 16 h/d seedling strengthening culture medium: MSB+0.8% agar+3% glucose pH=7 illumination 16 h/d (into the last three culture media, Kanamycin 0-50 mg/L L and cephalosporin 0-300 mg/L were added at the same time)

2. Agrobacterium infected transformation and plant regeneration

The somatic cell embryo masses of soybean with the diameters around 3 mm were placed in the prepared Agrobacterium infection liquor for infection. Then, the bacterial solution was poured away, and the sterile filter paper was used to absorb the redundant liquid to dry the embryo masses. Thereafter, the embryo masses were inoculated onto the co-culture medium, then onto the sterilization screening culture medium containing 50 mg/L of Kanamycin and 300 mg/L of cephalosporin (the concentrations decreased in sequence depending upon the situation, with the proviso that no bacteria grew). The infection time was 10 min. The co-culture time was 2 to 3 days. Acetosyringone was 100 μmol/L. The Agrobacterium concentration OD600 was 0.5-0.7. Subculturing was performed every 15 to 20 days. The number of the resistant somatic cell embryo masses (with the diameters around 3 mm) as generated was inspected within 3 months. The transformation ratio (the number of the resistant somatic cell embryo masses/the number of the inoculated somatic cell embryo masses×100) was calculated. Then, the resistant somatic cell embryo masses were transferred into the germination culture medium 1, and then into the germination culture medium 2 after 20 days of germination. Till the regenerated resistant small plants were grown, said plants were transferred into the seedling strengthening culture medium to obtain the transformed plants.

Genetic Transformation of Alfalfa

1. Materials

Alfalfa variety; Gongnon-1; Agrobacterium: LBA4404; a plant binary expression vector pCAMBIA2300 into which the HF gene was cloned and resistant to Kanamycin.

The culture medium was a MS culture medium added with various growth regulating substances, with a pH value of about 5.8. The culture temperature was 23 to 25° C. The illumination intensity was 2 000 1×; the illumination time was 18 h/d. The subculturing was performed about every 20 d.

2. Preparation of calluses

The hypocotyls were used as explants to undergo callus induction, and somatic embryo differentiation. After the somatic embryos were mature, somatic embryos were transferred into MS₀ for germination test.

3. Suspending culture of embryogenic calluses

3 g of calluses were inoculated into a 150 mL erlenmeyer flask containing 40 mL of suspending culture solution for performing suspending culturing. A fresh culture medium was used for change every 7 d. The rotational speed of the shaker was 150 r/min. Natural scattering light was used for illumination. After 15 d, the cell growth speed was determined. The suitable calluses were inoculated into the best embryogenic callus induction broth that had been screened out. The rotational speed of the shaker was set as 120 r/min. A fresh culture medium was used for change every 7 d. The illumination with natural scattering light lasted about 30 d.

4. Agrobacterium Transformation

Embryogenic calluses were placed in a 2.0 mL small centrifuge tube containing 600 μL of liquid co-culture medium for the ultrasonic wave treatment of 8 s with a parameter of 100m Hz and the subsequent co-culture of 4 d. The infected suspending embryogenic calluses were placed flatwise in a semi-solid co-culture medium containing 100 μmol/L of acetosyringone for dark culture of 4 d.

5. Screening and regeneration of transformed plants

The co-cultured embryogenic calluses were inoculated into the differentiation culture medium for culturing of 50 to 60 d. After 4 embryonic stages, embryogenic calluses grew into mature somatic embryos. Then, they were transferred into a somatic embryo germination culture medium. After about 20 to 30 d, when the plants grew to about 10 cm, the seedlings were transplanted, wherein the used Kanamycin screening concentration was 30 mg/L.

Genetic Transformation of Rape

1. Materials

Cabbage type rape variety CY2 for genetic transformation; Agrobacterium strain EHA105; a plant binary expression vector pCAMBIA1301 into which the HF gene was cloned.

2. Agrobacterium Transformation

Fresh bacterial colonies were selected by toothpick to be cultured in a YEB broth containing Km 50 mg/L and Rif 50 mg/L under shaking at 28° C., till logarithm dividing middle stage (OD600=0.3). The bacterial solution was taken for centrifugation at 12 000 r/min for 1 min, washed once with MS culture medium under centrifugation, and then diluted by 10 times. The recipient parent CY2 seeds were sterilized and inoculated onto a 1/2 MS culture medium for culturing sterile seedlings. After 5-7 d, hypocotyls were cut into small sections about 1 cm long to serve as explants for the Agrobacterium tumefaciens mediated transformation with the plasmid pCAMBIA1301 carrying HF gene. The transformation was carried out following the method of Wang Fulin et al. (Journal of Nuclear Agricultural Sciences, 5(26): 1129-1134(2011)). Transformants were screened by hygromycin (Hyg) 10 mg/L. The screened Hyg resistant seedlings rooted, and were domesticated in greenhouse pots for a period of time, and then transplanted into fields.

Genetic Transformation of Cotton

1. Materials and reagents

Cotton variety: Zhong 521; Agrobacterium strain GV3101; a plant binary expression vector pCAMBIA2300 into which the HF gene was cloned and resistant to Kanamycin.

MBS culture medium: MS inorganic ingredient+B5 organic ingredient as the basic culture medium, added with different hormone ingredients;

Infection liquor: MS inorganic salts+B5 organics+0.1 mg/L 2,4-D+0.1 mg/L KT+100 μmol/LAS (acetosyringone)+30 g/L glucose;

Co-culture: MS inorganic salts+B5 organics+0.1 mg/L 2,4-D+0.1 mg/L KT+100 μmol/LAS (acetosyringone)+30 g/L glucose+2.5 g/L plant gel;

Screening culture medium: MS inorganic salts+B5 organics+0.1 mg/L 2,4-D+0.1 mg/L KT+30 g/L glucose+2.5 g/L plant gel+Kanamycin 50 mg/L+150 mg/L carbenicillin

2. Culturing of explants

The cotton seeds delinted with concentrated sulfuric acid were cleaned with tap water; seed kernels were taken out. Then, the delinted seeds were placed into a sterilized erlenmeyer flask on a super-clean operating desk. The seeds were soaked with 70% to 75% alcohol for 1 min, rinsed with sterilized water, and then soaked with 2% sodium hypochlorite for 60 min. Thereafter, sodium hypochlorite was poured away, and the seeds were rinsed with sterilized water for many times, and soaked in sterilized water for 24 h. After the seeds were revealed, the seed coats were peeled off. The seeds were inoculated into a 1/2 MS seedling culture medium for dark culture at 28° C. The seedlings at the age of 5 d or so were taken to be cut into small pieces of 0.5-0.6 cm to serve as explants.

3. Co-culture of explants and Agrobacterium

Hypocotyls of sterile seedlings were cut into small sections of 0.5 cm or so, and soaked in Agrobacterium solution for 30 to 40 min. Sterile filter paper was used to absorb the bacterial solution. Said small sections were placed on a MSB solid culture medium for co-culture of 48 h.

4. Induction and selection of calluses and plant regeneration

The co-cultured hypocotyl cuts were transferred into the MSB solid screening culture medium containing 50 mg/L of kanamycin and 500 mg/L of carbenicillin. Till the culture lasted 60 d, the positive callus masses resistant to Kanamycin were selected to be transferred into the above culture medium free of antibiotic for subculturing. Thereafter, according to the state of calluses, particulate embryogenic calluses were obtained by adjusting the hormone concentration in the culture medium, and then embryoids were differentiated to culture regenerated plants.

Genetic Transformation of Wheat (Embryogenic Calluses)

1. Test materials

Immature embryo tissues were used for culturing. The test variety was Henong 827. Agrobacterium strain C58. A plant binary expression vector pCAMBIA2300 into which the HF gene was cloned and resistant to Kanamycin.

The culture media used in the genetic transformation process of wheat included:

Callus induction culture medium MSW0: MS basic medium+2 mg/L 2,4-D+4 mg/L picloride+0.5 g/L glutamine+0.75 g/L MgCl₂+0.1 g/L hydrolyzed casein+1.95 g/L MES+100 mg/L ascorbic acid+40 g/L maltose+4.5 g/L agar, pH 5.8;

Infection liquor PCM: MS basic medium+2 mg/L 2,4-D+4 mg/L picloride+0.5 g/L glutamine+0.75 g/L MgCl₂+0.1 g/L hydrolyzed casein+1.95 g/L MES+100 mg/L ascorbic acid+200 μmol/L acetosyringone+40 g/L maltose+4.5 g/L agar, pH 5.8;

Callus screening culture medium SM: MS basic medium+2 mg/L 2,4-D+4 mg/L picloride+0.5 g/L glutamine+0.75 g/L MgCl₂+0.1 g/L hydrolyzed casein+1.95 g/L MES+100 mg/L ascorbic acid+250 mg/L carbenicillin+25 mg/L G418+40 g/L maltose+4.5 g/L agar, pH 5.8;

Resistant callus differentiation culture medium RSM: MS basic medium+2 mg/L 2,4-D+4 mg/L picloride+0.5 g/L glutamine+0.75 g/L MgCl₂+0.1 g/L hydrolyzed casein+1.95 g/L MES+100 mg/L ascorbic acid+250 mg/L carbenicillin+25 mg/L G418+0.5 mg/L kinetin+0.2 mg/L naphthalene acetic acid+40 g/L maltose+4.5 g/L agar, pH 5.8;

2. Sterilization of immature grains and inoculation of immature embryos

The immature grains were taken 12 to 15 days after pollination of wheat to be surface-sterilized with 70% alcohol for 30 s, sterilized with 0.1% mercuric chloride for 8 min, and cleaned with sterilized water for 4-5 times. Immature embryos were picked out with dissecting needles, and were respectively inoculated onto the callus induction culture medium MSW0 with scutum upwards, for dark culture of 2 weeks at 25° C., and then transferred into the differentiation culture medium for illumination of 16 h at 25° C. and dark culture of 8 h for 4-6 weeks.

3. Agrobacterium-mediated genetic transformation procedures

The Agrobacterium C58 containing HF was inoculated uniformly with applicator onto the LB solid culture medium (pH 7.0, containing 50 mg/L of kanamycin and 50 mg/L of rifampicin) for culturing of 3 d at 28° C. and then culturing of 1 d at 23° C. Thereafter, a minor amount of Agrobacterium was scraped from the culture medium to be transferred and inoculated into the YEP broth containing the aforesaid antibiotic for overnight culture at 28° C., at the shaker rotational speed of 250 r/min.

Agrobacterium was collected till OD600 reached 1.0, and was re-suspended with PCM infection liquor. The re-suspension was used to soak calluses for 3 h. Then, the bacterial solution was poured away. The calluses were transferred into the culture dish spread with sterile filter paper for co-culture of 3 d, then transferred into the screening culture medium for dark culture of 2 weeks at 25° C., and then transferred into the differentiation culture medium for illumination culture at 25° C.

Genetic Transformation of Millet

The same method as wheat was used.

Genetic Transformation of Flax

1. Materials

Flax: Heiya 7; Agrobacterium tumefaciens strain EHA105; a plant binary expression vector pCAMBIA1301 into which the HF gene was cloned and resistant to Kanamycin.

2. Preparation of explants

Filled and shiny seeds Heiya 7 were selected, soaked with 75% alcohol for 5 min, soaked with 20% bleach powder supernatant for 20 min, rinsed with sterilized water for three times, and then inoculated onto the MS culture medium for dark culture of 5-7 d at 25° C. 2 days before application, the seeds were placed under illumination for 16 h each day at 22° C. for use.

3. Preparation of Agrobacterium bacterial solution

The propagation of strain EHA105 containing the gene of interest was performed using a YEP culture medium, peptone 10 g/L, yeast extract 10 g/L, NaCl 5 g/L, and kanamycin 50 mg/L. After inoculation, shaking culture was carried at 28° C. for 2 d. Top phase was removed by centrifugation for 10 min at 3000 r/min. The bacteria was suspended with a 1/2 MS broth (OD600=0.5) for transformation.

4. Selective pressure test

The sterile flax hypocotyls were cut into small pieces of 0.3-0.5 mm. Said small pieces were soaked with sterilized water for 10 min, absorbed dry by sterile filter paper, and respectively inoculated onto the MS culture medium of kanamycin 50 mg/L for culture at 24-26° C. The illumination period was 16 h each day.

5. Co-culture

The flax hypocotyls were cut into small pieces of 0.3-0.5 mm. Said small pieces were soaked with Agrobacterium EHA105 suspension for 10-20 min, absorbed dry by sterile filter paper, and respectively inoculated onto the MS, B5 or N6 culture medium of KT 2 mg/L, IAA 3.5 mg/L or HL 150 mg/L. The culture conditions were the same as above.

6. Screening culture and rooting

The screening culture medium was the same as that for co-culture, and only differed in the addition of 50 mg/L of kanamycin and 1000 mg/L of cephalosporin. The explants co-cultured for 3 days with Agrobacterium were soaked with 2000 mg/L of cephalosporin solution for 10-20 min, absorbed dry by sterile filter paper, and then inoculated onto the screening culture medium for culture under the same conditions as shown above. The sterilization and callus formation were inspected one week and two weeks after inoculation respectively. The selected resistant buds were transferred onto the rooting culture medium for induced rooting.

Genetic Transformation of Sunflower

1. Materials

H elianthusannuus Xinkuiza 6; Agrobacterium tumefaciens strain EHA105; a plant expression vector pCAMBIA1301 into which the HF gene was cloned.

2. Strain culturing

Fresh Agrobacterium tumefaciens single colonies were selected to inoculate into a YEP (1% yeast extract+1% tryptone+0.5% beef extract) broth under shaking at 28° C. overnight. On the next day, they were transferred and inoculated into a 20 mL YEP broth containing antibiotic at 1% inoculation amount for the further vibration and culture till logarithm growth period; bacteria were collected by centrifugation and diluted by MES liquid till OD₆₀₀ reached 0.8 as the working concentration for use.

3. Culture media

MS₀ medium: MS basic ingredients+2% sucrose+0.8% agar, pH 5.8;

GBA basal medium: MS₀+0.5 mg/L BA P+0.25 mg/L IAA+0.1 mg/L GA₃+30 g/L sucrose+0.8% agar, pH 5.8;

Co-culture medium (M C): GBA+acetosyringone (A CS) (100 m ol/L)+30 g/L sucrose+0.8% agar, pH 5.8;

Screening culture medium (M B): GBA+Carb 400 mg/L+hygromycin 10 mg/L+30 g/L sucrose+0.8% agar, pH 5.8;

Rooting medium (M R): 1/2M S₀+0.2 mg/L N A A+250 mg/L Carb+5 mg/L hygromycin+30 g/L sucrose+0.8% agar, pH 5.8.

4. Preparation of explants

The seeds that were filled, uniform in size and had no pests and diseases were selected, decorticated, soaked with 70% ethanol for 1 min, rinsed with sterilized water twice, sterilized with 1% AgNO₃ for 3 min, and rinsed with sterilized water for three times. The seeds were sowed onto a MS₀ solid culture medium and sprouted in dark at 28° C.; sterile seedlings were obtained after culture for 36-48 h. Roots, cotyledons and phyllopodiums of sterile seedlings were cut to reveal stem tips, and then cut longitudinally. The obtained explants contained a half of stem tip meristems and two halves of cotyledon axillary buds.

5. Infection

The prepared stem tip explants were soaked in bacterial solution sufficiently for 10 min, and then taken out. The sterile filter paper was used to absorb sufficiently the redundant bacterial solution on the surfaces of explants. The explants were placed onto a MC co-culture medium for co-culture of 3 d in dark at 28° C., and control was provided.

6. Transformant screening and plant regeneration

The explants co-cultured for 3 d were transferred onto a screening culture medium MB containing 10 mg/mL hygromycin (Hyg) for culture of 2 weeks, and then screened for 2-3 turns (2 weeks for each turn). The selected resistant buds were transferred onto the rooting culture medium MR for induced rooting.

Genetic Transformation of Taraxacum Kok-Saghyz Rodin (also Called Russian Dandelion)

1. Materials

Taraxacum kok-saghyz Rodin; Agrobacterium strain: GV3101; plasmid (pCAMBIA2300-35S-HF) which was a binary vector pCAMBIA2300 carrying the HF gene and resistant to Kanamycin.

2. Genetic transformation and regeneration of Taraxacum kok-saghyz Rodin

-   -   (1) Tissue-cultured seedlings growing well were selected. The         edges of the leaves were removed. The stem of Taraxacum         kok-saghyz Rodin was cut into a length of 2 cm. The leaves were         cut into the size of 1 cm². They were placed onto a MS culture         medium added with plant hormones 6-BA and NAA for dark culture         of 2 d;     -   (2) 200 μl was taken from Agrobacterium GV3101 glycerin tube         stored at −70° C. and containing plasmid pCAMBIA2300-35S-HF to         be inoculated into 50 ml of LB (50 mg/L Gen+100 mg/L Rif+50 mg/L         Kan) liquid for culture overnight;     -   (3) The bacterial solution cultured overnight was streaked on         the LB (50 mg/L Gen+100 mg/L Rif+50 mg/L Kan) solid culture         medium, placed upside down, for culture of 2 d at 28° C.;     -   (4) Monoclonal colonies were selected for inoculation onto the         LB (50 mg/L Gen+100 mg/L Rif+50 mg/L Kan) broth, for shaking         culture of 2 d at 28° C.;     -   (5) The cultured bacterial solutions were respectively         inoculated into 100 ml of LB (50 mg/L Gen+100 mg/L Rif+50 mg/L         Kan) liquid at a ratio of 1:100 for enlarged culture, and         activated till OD260 of about 0.6 for infection;     -   (6) The aforesaid two bacterial solutions were respectively         placed into 2 50 ml sterile large centrifuge tubes, and         centrifuged for 10 min at 5000 rpm;     -   (7) The supernatant was discarded. The bacteria was suspended by         100 ml of MS broth, and cultured for 5 min at 28° C.;     -   (8) The above explants cultured in dark for 2 d were placed into         the selected bacterial solution for shaking culture of 20 min at         28° C.;     -   (9) The infected explants were spread on the sterile dry filter         paper, with the redundant bacterial solution absorbed, for dark         culture of 2 d;     -   (10) After 2 d, the explants were taken out and placed onto the         MS (1 mg/L 6-BA+0.1 mg/L NAA+400 mg/L Cb (carbenicillin)+50 mg/L         Kan (Kanamycin)) solid culture medium; the plate was poured         every half a month;     -   (11) When adventitious shoots grew to 2 cm, single shoots were         broken off and inserted into the rooting culture medium 1/2 MS         (0.2 mg/L NAA+50 mg/L Kan+400 mg/L Cb) for growing;     -   (12) After one month, the strong tissue-cultured seedlings were         domesticated for 1 d, transplanted into nutrient soil (turfy         soil: vermiculite=3:1), covered with film for 1 week, and placed         in cultivation room for subsequent culturing.

Genetic Transformation of Maize

1. Materials and reagents Maize variety: Qi 319; Agrobacterium strain: GV3101; plasmid (pCAMBIA2300-35S-HF) which was a binary vector pCAMBIA2300 carrying the HF gene and resistant to Kanamycin.

D-culture medium: NaFeEDTA 10 ml/L+N6 macroelements 50 ml/L+B5 microelements 10 ml/L+Di comba (2,4-D) 1 ml/L (5 ml/L)+RTV 10 ml/L+Casamina acids (casein hydrolase) 0.5 g/L+L-Prine 700 mg/L+inositol 100 mg/L+Sucrose 20 g/L, pH 5.8

D-Inf culture medium: NaFeEDTA 10 ml/L+N6 macroelements 50 ml/L+B5 microelements 10 ml/L+Di comba (2,4-D) 1 ml/L+RTV 10 ml/L+Casamina acids (casein hydrolase) 0.5 g/L+L-Prine 700 mg/L+inositol 100 mg/L+Sucrose 68.5 g/L+glucose 36 g/L, pH 5.2

D-AS culture medium: D-culture medium+glucose 10 g/L+agar powder 8 g/L+AS (0.5 M) 200 μl+AgNO₃ 1 ml/L (both AS and AgNO₃ had the final concentration of 100 μM, and were added after sterilization of the culture medium when being slightly cool for uniform mixing)

D-Cef culture medium: D-culture medium+1 ml/L AgNO₃+cef 1 ml/L

2. Genetic transformation and regeneration of maize

-   -   (1) Preparation of maize immature embryo: maize leaves, maize         silks and some redundant parts were peeled off; a knife was         inserted into the upper portion for adding 70% ethanol; the         maize entered the super-clean operating desk; 30 s later, it was         taken out and blown dry on the super-clean operating desk for         about 15-20 min; 2/3 of the surface of the grain was peeled off;         immature embryo was peeled out.     -   (2) The bacterial solution added into D-Inf (containing AS) was         diluted till OD600 of 0.3-0.5 and stood for more than 1 h. The         immature embryo was washed once with D-Inf (free of AS), and         then soaked into the bacterial solution, upside down with hand         for 30 s, and stood for 5 min. Observed with no apparent wounds,         the immature embryo was taken out, absorbed dry with sterile         filter paper, and placed onto the D-AS solid culture medium for         co-culture of 3 d in dark at 25° C.     -   (3) Stage of restoring culture: the immature embryo co-cultured         for 3 d was rinsed in sterilized water (added with 1%₀ of cef)         for three times, 20 min for each time, and then absorbed dry         with filter paper, and transferred onto the D-Cef solid culture         medium, and restoring cultured in dark at 25° C. for 7 d.         Thereafter, pressurization screening stage was performed: in 4         cycles, with the interval of 2 weeks between any two.

The 1^(st) cycle: D culture medium+cef (1%₀)+PPT (5 mg/ml)

The 2^(nd) cycle: D culture medium+cef (1%₀)+PPT (10 mg/ml)

The 3^(rd) cycle: D culture medium+cef (1%₀)+PPT (10 mg/ml)

The 4^(th) cycle: D culture medium+cef (1%₀)+PPT (10 mg/ml)

-   -   (4) Restoration stage after screening: D culture medium+6-BA (5         mg/L), wherein 2,4-D or Dicamba concentration was diluted by 5         times, and sucrose was 30 g/L (or sucrose 20 g/L, glucose 10         g/L); the period was 2 weeks; dark culture.     -   (5) Induction stage after screening: D culture medium+6-BA (5         mg/L), wherein 2,4-D or Dicamba concentration was diluted by 5         times, and sucrose was 50 g/L, without the addition of glucose,         +cef 1 ml/L; dark culture.     -   (6) Differentiation stage: D culture medium, yet without the         addition of any hormone; sucrose concentration was 30 mg/L,         without the addition of glucose, +cef 1 ml/L; illumination         culture.     -   (7) Rooting stage: 1/2 MS culture medium.

Genetic Transformation of False Flax (Camelina Sativa) (by a Flower Dripping Method)

1. Materials and reagents

Camelina sativa; Agrobacterium strain: GV3101; plasmid (pCAMBIA2300-35S-HF) which was a binary vector pCAMBIA2300 carrying the HF gene and resistant to Kanamycin.

2. Genetic transformation of Camelina sativa by a flower dripping method

-   -   (1) Wild-type Camelina sativa was sowed in nutrient soil         (humus:vermiculite:perlite=4:2:1), 5 grains/pot (diameter: 9         cm), and placed in cultivation room for culturing. The         cultivation room had the temperature of 16 to 20° C. and the         relative humidity of 60%. The illumination intensity was 4 000         l×. The illumination period was 16 h illumination/8 h dark. When         the main stem of Camelina sativa plant grew to 5 cm and the         lateral branches were just bud-like, the top inflorescences were         removed to promote the growth and development of secondary         branches. When the plants grew to the full-bloom stage, they         were prepared for transformation. 2 d before transformation, the         formed fruit pods were cut off.     -   (2) When Agrobacterium GV3101 containing the plasmid         pCAMBIA2300-35S-HF was cultured till the OD600 value was 0.8, it         was infiltrated isometrically into the culture medium (1/2 MS,         5% sucrose, 200 μL/L Silwet L-77) to re-suspend bacteria and         transform Camelina sativa. Upon transformation, a pipettor was         used to suck Agrobacterium re-suspension for infiltration into         the culture medium and dripping onto the flower buds of Camelina         sativa, ensuring that each flower bud was dripped. Thereafter,         preservative films were used to coat the transformed plants to         maintain humidity. The plants stood upright in dark in the         cultivation room for culture of 1 d, and then were cultured         under normal conditions.     -   (3) After the plants were mature, the seeds were collected and         designated as T0 generation seeds. 50 mg/L of kanamycin was used         to screen the obtained T0 generation Camelina sativa seeds to         obtain positive transgenic plants.

The yield and biomass of the transgenic plants comprising the nucleic acid encoding the FTO obtained from the above methods and the control plants that do not comprise FTO were measured. The results are shown in table 2.

TABLE 2 Changes of the yield and biomass after the nucleic acid encoding the FTO were introduced into a variety of plants Biomass (fresh weight of the overground parts Plant (Organs Yield after removing for evaluating Increased the seeds) gene the yield) folds Increased folds Human maize (seed) 4.12 2.81 FTO soy bean (seed) 4.00 2.75 (SEQ tobacco (leaf) 3.65 2.54 ID potato (tuber) 3.83 2.61 NO: 5) alfalfa (stem and leaf) 2.43 2.43 rape (seed) 4.21 2.94 Russian dandelion 3.25 2.88 (Taraxacum kok-saghyz) (rubber solution in the root) cotton (seed cotton) 3.91 2.67 wheat 3.78 2.58 millet (seed) 4.08 2.79 flax (for oil) (seed) 3.77 2.58 sunflower (seed) 3.88 2.69 false flax (seed) 4.09 2.79 From table 2, it can be seen that after FTO was introduced into a variety of plants, the yield and the biomass were increased. 

The invention claimed is:
 1. A potato plant expressing a protein having an amino acid sequence selected from SEQ ID NOs: 1-4, wherein the plant produces a yield of tubers about four or more fold of that of the average yield of control plants grown under comparable conditions, wherein the control plants do not express the protein.
 2. The plant of claim 1, wherein the plant expresses a protein having an amino acid sequence of SEQ ID NO:
 1. 3. The plant of claim 1, wherein the plant expresses a protein having an amino acid sequence of SEQ ID NO:
 2. 4. The plant of claim 1, wherein the plant expresses a protein having an amino acid sequence of SEQ ID NO:
 3. 5. The plant of claim 1, wherein the plant expresses a protein having an amino acid sequence of SEQ ID NO:
 4. 6. A tobacco plant expressing a protein having an amino acid sequence selected from SEQ ID NOs: 1-4, wherein the plant produces a yield of leaves about four or more fold of that of the average yield of control plants grown under comparable conditions, wherein the control plants do not express the protein.
 7. The plant of claim 6, wherein the plant expresses a protein having an amino acid sequence of SEQ ID NO:
 1. 8. The plant of claim 6, wherein the plant expresses a protein having an amino acid sequence of SEQ ID NO:
 2. 9. The plant of claim 6, wherein the plant expresses a protein having an amino acid sequence of SEQ ID NO:
 3. 10. The plant of claim 6, wherein the plant expresses a protein having an amino acid sequence of SEQ ID NO:
 4. 